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质粒pIP501复制区域内转录的体外和体内分析。

In vitro and in vivo analysis of transcription within the replication region of plasmid pIP501.

作者信息

Brantl S, Nuez B, Behnke D

机构信息

Institute for Molecular Biology, Jena, FRG.

出版信息

Mol Gen Genet. 1992 Jul;234(1):105-12. doi: 10.1007/BF00272351.

Abstract

Derivatives of the conjugative streptococcal plasmid pIP501 replicate stably in Bacillus subtilis. The region essential for replication of pIP501 has been narrowed down to a 2.2 kb DNA segment, the sequence of which has been determined. This region comprises two genes, copR and repR, proposed to be involved in copy control and replication. By in vitro and in vivo transcriptional analysis we characterized three active promoters, pI, pII and pIII within this region. A putative fourth promoter (pIV) was neither active in vitro nor in vivo. We showed that copR is transcribed from promoter pI while the repR gene is transcribed from promoter pII located just downstream of copR. The pII transcript encompasses a 329 nucleotide (nt) long leader sequence. A counter transcript that was complementary to a major part of this leader was found to originate from a third promoter pIII. The secondary structure of the counter transcript revealed several stem-loop regions. A regulatory function for this antisense RNA in the control of repR expression is proposed. Comparative analysis of the replication regions of pAM beta 1 and pSM19035 suggested a similar organization of transcriptional units, suggesting that an antisense RNA is produced by these plasmids also.

摘要

接合性链球菌质粒pIP501的衍生物可在枯草芽孢杆菌中稳定复制。pIP501复制所必需的区域已缩小至一个2.2 kb的DNA片段,其序列已确定。该区域包含两个基因,copR和repR,推测它们参与拷贝控制和复制。通过体外和体内转录分析,我们对该区域内的三个活性启动子pI、pII和pIII进行了表征。一个假定的第四个启动子(pIV)在体外和体内均无活性。我们发现copR由启动子pI转录,而repR基因由位于copR下游的启动子pII转录。pII转录本包含一个329个核苷酸(nt)长的前导序列。发现一个与该前导序列大部分互补的反义转录本源自第三个启动子pIII。反义转录本的二级结构显示出几个茎环区域。推测该反义RNA在repR表达调控中具有调节功能。对pAMβ1和pSM19035复制区域的比较分析表明转录单元的组织方式相似,这表明这些质粒也产生反义RNA。

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